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从玻璃化冷冻的人类胚胎中获取人类胚胎干细胞系。

Derivation of human embryonic stem cell lines from vitrified human embryos.

作者信息

Peura Teija T, Schaft Julia, Stojanov Tomas

机构信息

Australian Stem Cell Centre QLD, Brisbane, Australia.

出版信息

Methods Mol Biol. 2010;584:21-54. doi: 10.1007/978-1-60761-369-5_2.

Abstract

Human embryonic stem cell lines are usually derived from human embryos that have become excess to clinical needs in assisted reproduction programs, whether because the couple in question has completed their family or because the embryo was found to be clinically unsuitable for transfer due to severe genetic condition (in case of pre-implantation genetic diagnosis, PGD). Culturing embryos to a blastocyst stage (5-6 days after IVF) before embryo transfer or cryopreservation instead of earlier commonly used 8-cell stage (3 days after IVF) calls for new methods for embryo cryopreservation and allows higher efficiencies for the actual stem cell derivation. Despite the vast advances in other fields of embryonic stem cell research, methods for derivation of new lines have not changed much over the years, mainly due to scarcity of embryos limiting experimentation. We describe here methods required to derive new embryonic stem cell lines starting from the initial cryopreservation of an embryo and finishing with a new cell line. We cover embryo cryopreservation and warming using a highly efficient vitrification method, the production of feeder cells and feeder plates, as well as embryo handling, plating and critical early passages, including earliest possible cryopreservation of putative stem cells using vitrification.

摘要

人类胚胎干细胞系通常源自辅助生殖项目中因临床需求过剩而多余的人类胚胎,这可能是因为相关夫妇已完成生育计划,或者是因为胚胎因严重遗传状况(如在植入前基因诊断,即PGD的情况下)被发现临床上不适合移植。在胚胎移植或冷冻保存之前将胚胎培养到囊胚阶段(体外受精后5 - 6天),而不是更早常用的8细胞阶段(体外受精后3天),这需要新的胚胎冷冻保存方法,并能提高实际干细胞衍生的效率。尽管胚胎干细胞研究的其他领域取得了巨大进展,但多年来新细胞系的衍生方法变化不大,主要是由于胚胎稀缺限制了实验。我们在此描述从胚胎的初始冷冻保存开始到新细胞系建立所需的方法。我们涵盖了使用高效玻璃化方法进行胚胎冷冻保存和复温、饲养细胞和饲养层板的制备,以及胚胎处理、接种和关键的早期传代,包括使用玻璃化对假定的干细胞尽早进行冷冻保存。

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